Cyclic lipopeptide acylase

ABSTRACT

The present invention provides a cyclic lipopeptide acylase which may effectively deacylate the acyl side chain of a cyclic lipopeptide compound, specifically FR901379 Substance or its analog thereof shown by the following general formula [I], and a process for production of a cyclic peptide compound which comprises the use of said acylase.                    
     [wherein R 1  is acyl; 
     R 2  is hydroxy or acyloxy; 
     R 3  is hydrogen or hydroxy; 
     R 4  is hydrogen or hydroxy; 
     R 5  is hydrogen or hydroxysulfonyloxy; and 
     R 6  is hydrogen or carbamoyl]

The present application is a Divisional Application of U.S. Ser. No.09/659,335, filed Sep. 12, 2000, now U.S. Pat. No. 6,372,474, which is aDivisional Application of U.S. Ser. No. 09/147,352, filed Dec. 31, 1998,now U.S. Pat. No. 6,146,872, which is a 371 application ofPCT/JP97/02003, filed Jun. 11, 1997.

TECHNICAL FIELD

This invention is concerned with an enzyme technology.

The present invention relates to a novel acylase which deacylates heacyl side chain of a cyclic lipopeptide compound and to a deacylationprocess comprising the use thereof.

More particularly, this invention relates to a novel acylase whichdeacylates the acyl side chain of FR901379 Substance, which is producedby Coleophoma sp. F-11899 (FERM BP-2635) (as described in Japanese KokaiTokkyo Koho H3-184921), or any analog of FR901379 Substance and to adeacylation process using the same.

BACKGROUND ART

There has been a standing demand for an acylase capable of deacylatingthe acyl side chain of a cyclic lipopeptide compound, specifically saidFR901379 Substance or an analog thereof, with good efficiency.

DISCLOSURE OF THE INVENTION

The inventors of this invention explored in earnest for a new acylasewhich might be able to deacylate the acyl side chain of a cycliclipopeptide compound represented by FR901379 Substance, Echinocandoin Band Aculeacin A, the latter two being analogs of FR901379 Substance. Asa result, they discovered an acylase in the fermentation broth availableupon culture of a certain filamentous fungus and succeeded in achievingthe objective deacylation with effectiveness.

The characteristics of the above novel cyclic lipopeptide acylase and ofthe deacylation process using the enzyme are now described in detail.

The cyclic lipopeptide acylase-producing strain of the invention isfirst described. The filamentous fungus as a novel cyclic lipopeptideacylase producer specifically includes but is not limited toOidiodendron sp. No. 30084, Oidiedendron echinulatum IFO 31963,Oidiodendron tenuissimum IFO 6798, Oidiodendron truncatum IFO 9951 andOidiodendron truncatum IFO 31812, all of which belong to the genusOidiodendron, and Verticillium sp. No. 30085 which belongs to the genusVerticillium.

The mycological characteristics of Oidiodendron sp. No. 30084 andVerticillium sp. No. 30085 are described below.

The fungus strain No. 30084 was isolated from a soil sample collected inJouhoku-machi, Higashi Ibaraki-gun, Ibaraki Prefecture. This strain crewrepressively on various media, forming colonies varying in color, e.g.greenish gray, brownish orange, yellowish white, etc., according todifferent kinds of culture media. On several media, strain No. 30084formed anamorphs showing a conidial structure consisting of a dendriticconidiophore rising up from the surface of the medium and arthroconidiaformed at its branches.

The detailed mycological characteristics of strain No. 30084 are asFollows.

The cultural characteristics of this fungus on various agar media aresummarized in Table 1. Colonies on malt extract agar crew regressivelyand spread to attain diameters from 1.5 to 2.0 cm after 2 weeks ofincubation at 25° C. The colony was circular and either raised as awhole or elevated peripherally and depressed in the center. The strainformed anamorphs in abundance, which presented with a powdery surface.The colony was greenish gray with a yellowish gray peripheral zone. Thereverse side was light yellow with a yellowish white peripheral zone. Onpotato dextrose agar, too, the colony grew repressively and spread toattain diameters from 1.5 to 2.0 cm under the same cultural conditionsas above. The surface of the colony was centrally elevated or convex,wrinkled, and somewhat felt-like, forming a small amount of anamorphs.The colony was brownish orange to light brown with an orange whiteperipheral zone. The reverse side was brown with an orange whiteperipheral zone.

The morphological characteristics of the strain was recorded byobserving its growth on Miura's medium (Miura, K. and M. Kudo: Trans.Mycol. Soc. Japan, 11: 116-118, 1970). The conidiophore of strain No.30084 stood erect from the surface of the medium and consisted of atan-colored linear trunk and colorless intricate branches. Thisdendritic structure made the conidiophore clearly distinguishable fromthe vegetative hypha. The conidiophore was 90 to 220 (or 240) μm inheight, with its trunk being 2 to 3 (or 3.5) μm wide. The ranches werebifurcated or trifurcated in succession and spread to occupy the space30 to 50 μm in height and 40˜60 μm in width over top of theconidiophore. Each branch was fragmented along a plurality of septae,forming conidia each in the form of a rod or an ellipsoid truncated atone end or both ends. The conidium was colorless, smooth-surfaced,unicellular, and varied in size from 2˜4×1.5˜2 μm. Individual conidiawere linked through vestiges of cell walls of the branch. The vegetativehypha was smooth-surface, septate, colorless, and branched. The hyphalcell was cylindrical and 1.0˜2.5 μm in width. No clamydospore wasobserved.

Strain No. 30084 was able to grow at 3 to 32° C. and the optimumtemperature for growth was 24 to 28° C. Those data were generated onpotato dextrose agar “Nissui” (Nissui Pharmaceutical).

The foregoing characteristics of strain No. 30084 were compared with thedescriptions in the taxonomic reference books on fungi such as (G. R.Barron: The Genera of Hyphomycetes from Soil, pp. 239-241, Williams &Wilkins, Baltimore, 1968), (J. A. von Arx: The Genera of Fungi,Sporulating in Pure Culture. pp. 180-184, J. Cramer, Vaduz, 1974) and(K. H. Domsch, W. Gams & T. H. Anderson: Compendium of Soil Fungi, pp.517-524, Academic Press, London, 1980). As a result, the abovecharacteristics were found to agree with the descriptions of the genusOidiodendron (Oidiodendron Robak 1932). Therefore, the strain wasidentified to be a strain belonging to the genus Oidiodendron and namedOidiodendron sp. No. 30084.

TABLE 1 Cultural characteristics of Strain No. 30084 Medium Culturalcharacteristics Malt extract agar* Growth: repressible, diameters1.5˜2.0 cm. Surface: circular, elevated to centrally concave, powdery,abundant anamorphs. Colonies are greenish gray (1B2-1C2) with ayellowish gray (4B2) peripheral zone. Reverse: pale yellow (4A3) with ayellowish white (4A2) peripheral zone. Potato dextrose agar Growth:repressible, diameters (Difco 0013) 1.5˜2.0 cm. Surface: circular,elevated to centrally convex, wrinkled, slightly felt-like, scantyanamorphs. Brownish orange (6C3) to light brown (6D6) with an orangishwhite (6A2) peripheral zone. Reverse: brown (7E6) with an orangish white(6A2) peripheral zone. Czapek's solution agar* Growth: very repressible,diameters 0.5˜1.0 cm. Surface: circular to amorphous, flat, powdery,abundant anamorphs. Greenish gray (29C2) with a light gray (1B1)peripheral zone. Reverse: Light gray (1B1) to greenish gray (25D2).Sabouraud's dextrose Growth: repressible, diameters agar medium 1.5˜2.0cm. (Difco 0190) Surface: circular, elevated to centrally convex,slightly felt-like, wrinkled. No anamorph formed. Grayish orange (6B3)to brownish orange (6C7), with an orangish white (6A2) peripheral zone.Reverse: light brown (6D6), with an orangish white (5A2) peripheralzone. Emerson YpSs Growth: very repressible, diameters agar medium0.5˜1.0 cm. (Difco 0739) Surface: circular, flat, no rise-up of aerialhypha. No anamorph formed. Yellowish white (4A2). Reverse: Yellowishwhite (4A2). Corn meal agar Growth: very repressible, diameters (Difco0386) 1.0˜1.5 cm. Surface: circular, flat, no rise-up of aerial hypha.Scanty anamorphs. White (1A1) to yellowish white (4A2). Reverse:yellowish white (4A2). MY20 agar* Growth: very repressible, diameters1.0˜1.5 cm. Surface: circular, elevated to convex, powdery, wrinkled.Abundant anamorphs. Greenish gray (27D2) in center, with a light gray(1B1) peripheral zone. Reverse: yellowish white (4A2) to pale yellow(4A3). *The compositions of malt extract agar, Czapek's solution agar,and MY20 agar are based on JCM Catalog (Nakase, T., 5th ed., 503 p.,Japan Collection of Microorganisms and Life Science Research InformationSection of the Institute of Physical and Chemical Research, Saitama,1992).

The above data are the results of observation after 14 days ofincubation at 25° C. The color descriptions are based on MethuenHandbook of Colour (Kornerup, A. and J. H. Wanscher, 3rd ed., 525pp.,Methuen, London, 1978).

This strain was originally deposited with National Institute ofBioscience and Human Technology (NIBH, Hiagashi 1-1-3, Tsukuba-shi,Ibaraki, Japan) (Zip code 305) and assigned with an accession number ofFERM P-15550 (date of acceptance: Apr. 2, 1996) but has been convertedto a deposit under Budapest Treaty on May 15, 1997 and assigned with anaccession number of FERM BF-5943.

The fungus strain No. 30085 was isolated from a soil sample collected inJouhoku-machi, Higashi Ibaraki-gun, Ibaraki Prefecture. This strain crewrepressively on various media, forming colonies varying in color, (e.g.greenish gray, yellowing gray, brown, etc.) and, on several media,produced brown soluble pigments diffusing into the medium. No sporogenicorgan was observed normally, but only after prolonged incubation on cornmeal agar “Nissui” (Nissui Pharmaceutical), this strain formed a minimalquantity of asexual spores.

The mycological characteristics of strain No. 30085 are as follows.

The cultural characteristics of the stain on various agar media aresummarized in Table 2. The colony on potato dextrose agar grewrepressively and spread to attain diameters from 2.0 to 3.0 cm after 2weeks of incubation at 25° C. The colony was circular, flat to elevated,slightly wrinkled and felt-like. An orange-colored exudate was observedon the surface of the colony. The colony was greenish gray to pale gray,with an orangish white to orangish gray peripheral zone. The reverseside was grayish brown to dark brown with a grayish orange peripheralzone and a diffusion of brown soluble pigments into the medium wasobserved. The colony on Czapek's solution agar grew much repressivelyand spread circularly to attain diameters 1.0˜2.0 cm after 2 weeks ofincubation at 25° C. The surface of the colony was flat and thin, withno rise-up of aerial hyphae. The surface color was white or yellowishgray, and the reverse color was the same.

The morphologic characteristics of strain No. 30085 were determinedaccording to the findings on said corn meal agar “Nissui”. Theconidiophore of strain No. 30085 was not clearly distinguishable fromthe vegetative and aerial hyphae, and 2˜5 conidiogenous cells occurredin whirl, or at times singly, at the side of the filament. Theconidiogenous cell was colorless, smooth-surface, filamentous toelongated flask-shaped (lecythiform), measuring 18 to 37 (45 attimes)×1.5 to 2 μm and forming a single conidium to several conidia in acontinuous series at the tip. The mode of conidiogenesis appeared to bephialidic but no definite collarette was observed. The conidium wascolorless, smooth-surfaced, prolate (ellipsoidal) to bacilliform(rod-shaped), unicellular and 3˜5.5×1.5˜2.5 μm in size. The vegetativehypha was smooth-surfaced, septate, colorless and branched, and althoughit was usually linear but at times curved and remarkably crimped. Thehyphal cell was cylindrical to filiform and 1.0˜5.0 μm in width,containing a large number of intracellular vacuoles. Those vaculoes wereleased extracellularly with aging of the cell to give a highly viscousexudate. The clamydospore, sclerotium and catenulate form(concatinations) were not observed, but in old culture, thepleurogenesis of a large number of globose cells was at times observed.

Strain No. 30085 was able to grow at 4˜29° C., and the optimumtemperature for growth was 22˜26° C. Those data were generated on potatodextrose agar (Nissui pharmaceutical).

The above characteristics of the strain were compared with thedescriptions in several books on the taxonomy of fungi, such as (G. R.Barron: The Genera of Hyphomycetes from Soil, pp. 364, Williams &Wilkins, Baltimore, 1968), (J. A. von Arx: The Genera of Fungi,Sporulating in Pure Culture. pp. 315, J. Cramer, Vaduz, 1974) and (K. H.Domsch, W. Gams & T. H. Anderson: Compendium of Soil Fungi, pp. 859,Academic Press, London, 1980). As a result, strain No. 30085 was foundto resemble Verticillium which is a fungus imperfecti (Verticillium Nees1816). Fungi of the genus Verticillium are different from strain No.30085 in that the former produce a large number of conidia as a mucoidmass at the tip of the phialide. Regarding this difference, it wasconsidered that strain No. 30085 was sole to form only one or a fewconidia because of its poor sporogenous ability. Based on the aboveobservation, the strain was identified as a species of the genusVerticillium and named Verticillium sp. No. 30085.

TABLE 2 Cultural characteristics of Strain No. 30085 Medium Culturalcharacteristics Malt extract agar* Growth: repressible, diameters2.0˜3.0 cm. Surface: circular, flat, felt-like to cottony. A pale orangeexudate is produced. The colony is pale gray (1B1) to light gray(1C1)-greenish gray (27F2), with an orangish white (5A2) peripheralzone. Reverse: dark green (28F to 4) with a yellowish white (4A2)peripheral zone. Potato dextrose agar Growth: repressible, diameters(Difco 3013) 2.0˜3.0 cm. Surface: circular, flat to elevated, slightlywrinkled, felt-like; an orange-colored exudate produced. Greenish gray(1B2) to pale gray (1B1) with an orangish white (6A2)-orangish gray(6B2) peripheral zone. Reverse: grayish brown (6F3) to dark brown (6F4to 5), with a grayish orange (5B3)-brown peripheral zone. Diffusion ofbrown soluble pigments was observed. Czapek's solution Growth: veryrepressible, agar* diameters 1.0˜2.0 cm. Surface: circular, flat, thin,no rise-up of aerial hyphae, white (1A1) or yellowish gray (2C2).Reverse: white (1A1) or yellowish gray (2C2) Sabouraud's dextroseGrowth: repressible, diameters agar medium 2.0˜2.5 cm. (Difco 0190)Surface: circular, elevated to centrally convex; the surface wetted byan exudate and glossy; somewhat wrinkled, and the aerial hyphae in thecenter were consolidated into a bundle. Yellowish gray (4B2) to grayishyellow (4B3) but light brown (6D4) in the center. Reverse: dark brown(7F6-7) with a brown (7E7) peripheral zone, with diffusion of brownsoluble pigments. Emerson YpSs Growth: repressible, diameters agarmedium 1.5˜2.5 cm. (Difco 0739) Surface: circular, flat to elevated,wrinkled, felt-like, gray with an olive tinge (2E2). Pale Gray (2B2) inthe peripheral zone. Reverse: dark brown (7F5-6) with a brown (7E5)peripheral zone. Diffusion of brown soluble pigments noted. Corn mealagar Growth: slightly repressible, (Difco 0386) diameters 2.5˜3.0 cm.Surface: circular, flat and thin, with no rise-up of aerial hyphae.Greenish gray (1B2-1C2) but olive (1F3) in the center. Reverse: greenishgray (1C2) but olive (1F3) in the center. MY20 agar* Growth: muchrepressible, diameters 0.5˜1.0 cm. Surface: circular, elevated toconvex, wetted by an exudate and glossy. The aerial hyphae in the centerwere consolidated into a bundle. Brown (6E4). Reverse: dark brown (6F5),with diffusion of brown soluble pigments.

The compositions of malt extract agar, Czapek's solution agar, and MY20agar are based on JCM Catalog Nakase, T., 5th ed., 503 p., JapanCollection of Microorganisms and Life Science Research InformationSection of the Institute of Physical and Chemical Research, Saitama,1992).

Those data were generated by observation after 14 days of incubation at25° C. after inoculation. The color descriptions are based on MethuenHandbook of Colour (Kornerup, A. and J. H. Wanscher, 3rd ed., 525pp.,Methuen, London, 1978).

This strain was originally deposited with National Institute ofBioscience and Human Technology (NIBH, Higashi 1-1-3, Tsukuba-shi,Ibaraki, Japan) (Zip code 305) and assigned with an accession number ofFERM F-15551 (date of acceptance: Apr. 2, 1996). It was initiallydesignated as Fugus No. 30085. However, the strain was renamedVerticillium sp. No. 30085 on Aug. 16, 1996 and converted to a depositunder Budapest Treaty on May 15, 1997 with assignment of an accessionnumber of FERM BP-5944.

Oidiodendron echinulatum IFO 31963, Oidiodendron tenuissimum IFO 6798,Oidiodendron truncatum IFO 9951 and Oidiodendron truncatum IFO 31812 aresubcultures allotted from Institute for Fermentation, Osaka 2-17-85 JusoHommachi, Yodogawa-ku, Osaka-shi).

The term “cylic lipopeptide compound” as used throughout thisspecification means a compound having a polypeptide ring and, as a sidechain located on the ring, an “acylamino group”, which substanceoptionally may have other side chains.

FR901379 Substance, which is a representative species of said “cycliclipopeptide compound”, is a known compound having antifungal activity asproduced by the microorganism Coleophoma sp. F-11899 (FERM BP-2635) (asdescribed in Japanese Kokai Tokkyo Koho H3-184921). It is a compound ofthe following chemical formula [Ia]:

The term “analog of FR901379 Substance” means any compound of thefollowing general formula [I] or a salt thereof.

[wherein R¹ is acyl;

R² is hydroxy or acyloxy;

R³ is hydrogen or hydroxy;

R⁴ is hydrogen or hydroxy;

R⁵ is hydrogen or hydroxysulfonyloxy; and

R⁶ is hydrogen or carbamoyl]

The novel cyclic lipopeptide acylase according to this invention is anacylase derived from a strain belonging to the genus Oidiodendron or thegenus Verricillum and capable of deacylating the side chain “acylamino”group of said cyclic lipopeptide compound to an “amino” group. To bespecific, said acylase is an enzyme which deacylates the palmitoyl sidechain of FR901379 Substance or a salt thereof or the acyl side chain ofthe analog of FR901379 Substance of general formula [I], inclusive ofFR901379 Substance, or a salt thereof to give the objective cyclicpeptide compound, specifically a compound of the following chemicalformula [IIa] (FR179642 Substance):

or a salt thereof, or an analog of FR179642 of the following generalformula [II] which includes FR179642 Substance:

[wherein R², R³, R⁴, R⁵, and R⁶ are the same groups as respectivelydefined above] or a salt thereof.

The preferred species of the above-mentioned salt of compound [I] and[II] are nontoxic mono- or di-salts of the conventional types, thusincluding metal salts for example alkali metal salts (e.g. sodium salt,potassium salt, etc.) and alkaline earth metal salts (e.g. calcium salt,magnesium salt, etc.), ammonium salts, salts with organic bases (e.g.trimethylamine salt, triethylamine salt, pyridine salt, picoline salt,dicyclohexylamine salt, N,N′-dibenzylethylenediamine salt, etc.),organic acid addition salts (e.g. formate, acetate, trifluorcacetate,maleate, tartarate, methanesulfonate, benzenesulfonate,toluenesulfonate, etc.), inorganic acid addition salts (e.g.hydrochloride, hydrobromide, hydroidide, sulfate phosphate, etc. andsalts with amino acids (e.g. arginine, aspartic acid, glutamic acid,etc.).

The preferred example of “lower alkyl” may include straight-chain orbranched-chain alkyl groups containing 1˜6 carbon atom(s), such asmethyl, ethyl, propyl, isopropyl, butyl, isobutyl, tert-butyl, pentyl,isopentyl and hexyl. The more preferred one may be C₁₋₄ alkyl, and thestill more preferred one may be methyl.

The preferred example of “higher alkyl” may include straight-chain orbranched-chain alkyl groups containing 7˜20 carbon atom(s), such asheptyl, octyl, 3,5-dimethyloctyl, 3,7-dimethyloctyl, nonyl, decyl,undecyl, dodecyl, tridecyl, tetradecyl, pentadecyl, hexadecyl,heptadecyl, octadecyl, nonadecyl and eicosyl.

The preferred example of “lower alkoxy” may include straight-chain orbranched-chain alkoxy groups such as methoxy, ethoxy, propoxy,isopropoxy, butoxy, isobutox, tert-butoxy, pentyloxy, tert-pentyloxy,neopentyloxy, hexyloxy and isohexyloxy.

The referred example of “higher alkoxy” may includes straight-chain ofbranched-chain groups such as neptyloxy, octyloxy, 3,5-dimethyloctyloxy,3,7-dimethyloctyloxy, nonyloxy, decyloxy, undecyloxy, docecyloxy,tridecyloxy, tetradecyloxy, hexadecyloxy, heptadecyloxy, octadecyloxy,nonadecyloxy and eicosyloxy.

The preferred example of “aryl” may include phenyl optionally havinglower alkyl (e.g. phenyl, mesityl, tolyl, etc.), naphthyl and anthryl,among others.

The “acyl” moiety of the preferred species of “acylamino” or “acyl” mayinclude aliphatic acyl groups derived from carboxylic acids, carbonicacids, carbamic acids, sulfonic acids, etc., aromatic acyl,heterocyclic-acyl, aryl-substituted aliphatic acyl, andheterocyclic-substituted aliphatic acyl.

The preferred examples of said “acyl” moiety may include aryl (e.g.phenyl, naphthyl, anthryl, etc.) which may have one or more (preferably1˜3) suitable substituent(s) such as halogen (e.g. fluoro, chloro,bromo, iodo), hydroxy, said higher alkoxy and said aryl; said loweralkoxy; amino; protected amino [preferably acylamino, such as loweralkoxycarbonylamino (e.g. methoxycarbonylamino, ethoxycarbonylamino,propoxycarbonylamino, butoxycarbonylamino, t-butoxycarbonylamino,pentyloxycarbonylamino, hexyloxycarbonylamino, etc.) etc.];di(lower)alkylamino (e.g. dimethylamino, N-methylethylamino,diethylamino, N-propylbutylamino, dipentylamino, dihexylamino, etc.);lower alkoxyimino (e.g. methoxyimino, ethoxyimino, propoxyimino,butoxyimino, t-butoxyimino, pentyloxyimino, hexyl-oxyimino, etc.; arlower)alkoxyimino such as phenyl(lower)alkoxyimino which may have one ormore (preferably 1˜3) suitable substituent (s) such as said higheralkoxy (e.g. benzyloxyimino, phenethyloxyimino, benzhydryloxyimino,etc.); heterocyclicthio (preferably pyridylthio) which may have one ormore (preferably 1˜3 suitable substituent(s) such as higher alkyl (e.g.heptyl, octyl, 2-ethylhexyl, nonyl, decyl, 3,7-dimethyloctyl, undecyl,dodecyl, tridecyl, tetradecyl, pentadecyl, 3-methyl-10-ethyldodecyl,hexadecyl, heptadecyl, octadecyl, nonadecyl, eicosyl, etc.); loweralkanoyl (e.g. formyl, acetyl, propionyl, butyryl, isobutyryl, valeryl,hexanoyl, pivaloyl, etc.) which may have one or more (preferably 1˜3)suitable substituents) such as heterocyclic group (e.g. thienyl,imidanolyl, pyrazoly, furyl, tetrazolyl, thiazolyl, thiadiazolyl, etc.;which, in turn, may have one or more (preferably 1˜3) suitablesubstituent(s) such as amino, said protected amino, said higher alkyl,etc.;

higher alkanoyl (e.g. heptanoyl, octanoyl, nonanoyl, decanoyl,undecanoyl, lauroyl, tridecanoyl, myristoyl, pentadecanoyl, palmitoyl,10,12-dimethyltetradecanoyl, heptadecanoyl, stearoyl, nonadecanoyl,eidosanoyl, etc.);

lower alkenoyl (e.g. acryloyl, methacryloyl, crotonyl, 3-pentenoyl,5-hexenoyl, etc.) which may have one or more (preferably 1˜3) suitablesubstituent(s) such as said aryl which, in turn, may have one or more(preferably 1˜3) suitable substituent(s) such as said higher alkoxy;

higher alkenoyl (e.g. 4-heptenoyl, 3-octenoyl, 3,6-decadienoyl,3,7,11-trimethyl-2,6,10-dodecatrienoyl, 4,10-heptadecadienoyl, etc.);

lower alkoxycarbonyl (e.g. methoxycarbonyl, ethoxycarbonyl,propoxycarbonyl, butoxycarbonyl, t-butoxycarbonyl, pentyloxycarbonyl,hexyloxycarbonyl, etc.);

higher alkoxycarbonyl (e.g. heptyloxycarbonyl, octyloxycarbonyl,2-ethylhexyloxycarbonyl, nonyloxycarbonyl, decyloxycarbonyl,3,7-dimethyloctyloxycarbonyl, undecyloxycarbonyl, dodecyloxycarbonyl,tridecyloxycarbonyl, tetradecyloxycarbonyl, pentadecyloxycarbonyl,3-methyl-10-ethyldodecyloxycarbonyl, hexadecyloxycarbonyl,heptadecyloxycarbonyl, octadecyloxycarbonyl, nonadecyloxycarbonyl,eicosyloxycarbonyl, etc.);

aryloxycarbonyl (e.g. phenoxycarbonyl, naphthyloxycarbonyl, etc.);

arylglyoxyloyl (e.g. phenylglyoxyloyl, napnthylglyoxyloyl, etc.;

ar(lower)alkoxycarbonyl which may have one or more suitablesubstituent(s), for example phenyl-(lower)alkoxycarbonyl which may havenitro or lower alkoxy (e.g. benzyloxycarbonyl, phenethyloxycarbonyl,p-nitrobenzyloxycarbonyl, p-methoxybenzyloxycarbonyl, etc.);

lower alkylsulfonyl (e.g. methylsulfonyl, ethylsulfonyl, propylsulfonyl,isopropylsulfonyl, pentylsulfonyl, butylsulfonyl, etc.);

arylsulfonyl (e.g. phenylsulfonyl, naphthylsulfonyl, etc.) which mayhave one or more (preferably 1˜3) suitable substituent(s) such as saidlower alkyl, said higher alkoxy, etc.;

ar(lower) alkylsulfonyl such as phenyl(lower)-alkylsulfonyl (e.g.benzylsulfonyl, phenethylsulfonyl, benzhydrylsulfonyl, etc.;

said halogen; lower alkyl (e.g. methyl, ethyl, propyl, butyl, t-butyl,pentyl, hexyl, etc.); said higher alkyl; lower alkoxy (e.g. methoxy,ethoxy, propoxy, butoxy, t-butoxy, pentyloxy, hexyloxy, etc.) which mayhave one or more (preferably 1˜10) suitable substituent(s) such as saidlower alkoxy, said halogen, said aryl, etc.; higher alkoxy (e.g.heptyloxy, octyloxy, 2-ethylhexyloxy, nonyloxy, decyloxy,3,7-dimethyloctyloxy, undecyloxy, docdecyloxy, tridecyloxy,tetradecyloxy, pentadecyloxy, 3-methyl-10-ethyl-dodecyloxy,hexadecyloxy, heptadecyloxy, octadecyloxy, nonadecyloxy, eicosyloxy,etc.) which may have one or more (preferably 1˜17) suitablesubstituent(s) such as said halogen; higher alkenyloxy (e.g.3-heptenyloxy, 7-octenyloxy, -2,6-octadienyloxy, 5-nonenyloxy,1-decenyloxy, 3,7-dimethyl-6-octenyloxy, 3,7-dimethyl-2,6-octadienyloxy,8-undecenyloxy, 3,6,8-dodecatrienyloxy, 5-tridecenyloxy,7-tetradecenyloxy, 1,8-pentadecadienyloxy, 15-hexadecenyloxy,11-heptadecenyloxy, 7-octadecenyloxy, 10-nonadecenyloxy,18-eicosenyloxy, etc.); carboxy; said aryl which may have one or more(preferably 1˜3) suitable substituent(s) such as said higher alkoxy;aroyl (e.g. benzoyl, napthoyl, anthrylcarbonyl, etc.) which may have oneor more (preferably 1˜5) suitable substituent(s) such as aryloxy (e.g.phenoxy, naphthyloxy, anthryloxy, etc.) which, in turn, may have one ormore preferably 1˜3) suitable substituent(s) such as, for example, saidlower alkoxy or said higher alkoxy; and so on.

Among the above-mentioned species of “acyl”, the preferred one may behigher alkanoyl, and the particularly preferred one may be palmitoyl.

The “acyl” moiety in the term of “acyloxy” can be referred toaforementioned “acyl”.

The preferred example of “acyloxy” may include lower alkanoyloxy (e.g.formyloxy, acetyloxy, propionyloxy, outyryloxy, isobutyryloxy,valeryloxy, hexanoyloxy, pivaloyvloxy, etc.) and phosphonoxy.

The acylase of this invention is one of the so-called inducible enzymes,and it is an essential requisite for she production of the enzyme that acyclic lipopeptide compound of formula [I], for example FR901379Substance, is present in the medium in the process of growth of thefungal producer of this acylase. Therefore, this acylase can be producedby culturing a fungal strain capable of producing this particularacylase, for example any of Oidiodendron sp. No. 30084, Oidiodendronechinulatum IFO 31963, Oidiodendron tenuissimum IFO 6798, Oidiodendrontruncatum IFO 9951 and Oidiodendron truncatum IFO 31812, all of whichbelong to she genus Oidiodendron, or Verticillium sp. No. 30085 whichbelongs to the genus Verticillium, in the presence of said cycliclipopeptide compound in a culture medium.

More particularly, the acylase can be produced by culturing saidacylase-producing fungal strain in a nutrient medium containing one ormore assimilable carbon sources and digestable nitrogen sources in thepresence of said cyclic lipopeptide compound of formula [I], for exampleFR901379 Substance, preferably aerobically by, for example, shakeculture or submerged culture.

Generally speaking, this novel acylase can be produced by culturing saidnovel acylase-producing fungus in an aqueous medium containingassimilable carbon and digestable nitrogen sources preferablyaerobically by shake culture or submerged culture.

The preferred source of carbon to be present in the culture medium mayinclude carbohyrates such as glucose, xylose, galactose, glycerol,starch and dextrin. As other sources of carbon, there may be mentionedmaltose, rhamnose, raffinose, arabinose, mannose, salicin, sodiumsuccinate, etc.

The preferred source of nitrogen may include yeast extract, peptone,gluten meal, cottonseed flour, soybean flour, corn steep liquor, driedyeast, wheat germ, feather powder, peanut flour, etc. and inorganic ororganic nitrogen compounds such as ammonium salts, (e.g. ammoniumnitrate, ammonium sulfate, ammonium phosphate, etc.), urea, amino acids,etc.

While those sources of carbon and nitrogen are preferably used insuitable combinations, it is not necessary to use pure sources, for evenmaterials of low purity can be used only provided that they containsuitable amounts of growth factors and reasonable amounts of inorganicnutrients. This is because impure materials sometimes contain suchgrowth factors and trace elements and, therefore, can be used withadvantage. Optionally, the medium may be suppplemented with sodiumcarbonate or calcium carbonate, sodium phosphate or potassium phosphate,sodium chloride or potassium chloride, sodium iodide or potassiumiodide, magnesium salts, copper salts, cobalt salts and other inorganicsalts. Particularly, when the culture medium produces a copious foam, anantifoam such as liquid paraffin, fatty oil, vegetable oil, mineral oilor silicone oil may be added as necessary.

For the high production of this novel acylase, submerged aerobic cultureis the preferred method. For small-scale production, shake culture orsurface culture in a flask or bottle is carried out. For culturing thefungus in a large tank, it is preferable to carry out a preculture andinoculate the production tank with the resulting seed culture in orderthat growth retardation of the fungus may be avoided. Thus, preferably arelatively small quantity of medium is inoculated with spores or hyphaeof the microorganism, and the inoculated medium is incubated to preparea seed culture in the first place, and the resulting seed culture isaseptically transferred to the large tank. The medium for use in thispreparation of a seed culture may be substantially identical to ordifferent from the medium or use in the production of the novel acylase.

The agitation and aeration of the fermentation broth can be achieved invarious ways. The agitation can be achieved by using a propeller mixeror the like stirring device, rotating or reciprocating a fermentationjar, using a pump of optional construction or blowing sterile airthrough the medium. The aeration can be achieved by passing sterile airthrough the fermentation system.

The fermentation is carried out at a temperature of generally about5˜32° C., preferably 20˜30° C., and a pH level of 6˜8 for about 50˜150hours, although those conditions may be varied according to otherconditions and scale of fermentation.

The novel acylase thus produced can be recovered from the fermentationbroth by the conventional procedures which are usually employed in therecovery of other known bioactive substances. The novel acylase thusproduced occurs in both the cultured mycelium and the supernatant of thebroth. Therefore, the novel acylase can be separated from the myceliumand the supernatant or filtrate available on filtration orcentrifugation of the fermentation broth and purified by theconventional procedures such as concentration under reduced pressure,freeze-drying, extraction with the common solvent, pH adjustment,treatment with a conventional resin such as an anion exchange resin, acation exchange resin, a nonionic adsorbent resin, or the like,treatment with a conventional adsorbent such as active charcoal, silicicacid, silica gel, cellulose, alumina, or the like, crystallization, and,recrystallization.

Referring to the level of addition of the cyclic lipopeptide compound ofthe formula [I], e.g. FP901379 Substance, which is necessary, forinducing production of the enzyme, the cyclic lipopeptide compound needbe available only in a minimal amount in the medium during the growth ofthe acylase-producing fungus and usually the objective effect can bewell obtained by adding about 0.01 to 1% of the substance to the culturemedium. It is not essential to add the cyclic lipopeptide to thepreculture medium.

In the fermentative production of FR901379 Substance, it is possible toinoculate the FR901379 production medium with an FR901379-producingstrain and said acylase-producing strain concurrently or at staggeredtimes so as to let FR179642 Substance be directly produced in the broth.

The following examples are intended to illustrate but by no meansdelimit the deacylation technology of the invention which comprises theuse of the acylases produced by the fungi Oidiodendron sp. No. 30084,Oidiodendron echinulatum IFO 31963, Oidiodendron tenuissimum IFO 6798,Oidiodendron truncatum IFO 9951, Oidiodendron truncatum IFO 31812 andVerticillium sp. No. 30085.

Process for production of the acylase

EXAMPLE-1-1

Production the acylase elaborated by Oidiodendron sp. No. 30084

As the preculture medium, a medium comprising glucose 1%, soluble starch2%, cottonseed flour 3%, soybean flour 1.5%, potassiumdihydrogenphosphate 1% and calcium carbonate 0.2% was used. As theproduction medium, a medium comprising glucose 6%, yeast extract 1% andpotassium dihydrogenphosphate 0.1% (adjusted to pH 6.0 beforesterilization) was used.

A 100-ml conical flask containing 30 ml of said preculture medium wassterilized by autoclaving at 120° C. for 20 minutes. After cooling toroom temperature, the flask was inoculated with 1˜2 loopfuls of a slantagar culture of Oidiodendron sp. No. 30084. After cooling to roomtemperature, shake culture was carried out at 25° C. for 7 days toprepare a seed culture. Then, a 500-ml conical flask containing 100 mlof said production medium was sterilized at 120° C. for 20 minutes andcooled to room temperature, and FR901379 Substance was aseptically addedat a final concentration of 0.1%. The flask was then inoculated with 2ml of said seed culture and incubated with shaking at 30° C. for 3 daysto provide an enzyme broth.

EXAMPLE 1-2

Production of the acylase elaborated by Verticillium sp. No. 30085

As the preculture medium, a medium comprising glucose 1%, soluble starch2%, cottonseed flour 3%, soybean flour 1.5%, potassium dihydrogenphosphate 1% and calcium carbonate 0.2% was used. As the productionmedium, a medium comprising glucose 6%, yeast extract and potassiumdihyadrogenphosphate 0.1% (adjusted to pH 6.0 before sterilization) wasused.

A 100-ml conical flask containing 30 ml of said preculture medium wassterilized by autoclaving at 120° C. for 20 minutes. After cooling toroom temperature, the flask was inoculated with 1≠2 loopfuls of a slantagar culture of Verticillium sp. No. 30085. After cooling to roomtemperature, shake culture was carried out at 25° C. for 7 days toprepare a seed culture. Then, a 500-ml conical flask containing 100 mlof said production medium was sterilized at 120° C. for 20 minutes andcooled to room temperature, and FR901379 Substance was aseptically addedat a final concentration of 0.1%. The flask was then inoculated with 2ml of said seed culture and incubated with shaking at 30° C. for 4 daysto provide an enzyme broth.

EXAMPLE 1-3

Production of the acylase elaborated by Oidiodendron tenuissimum IFO6798 allotted from Institute for Fermentation, Osaka 2-17-85,Juso-Hommachi, Yodogawa-ku, Osaka)

As the preculture medium, a medium comprising glucose 1%, soluble starch2%, cottonseed flour 3%, soybean flour 1.5%, potassiumdihydrogenphosphate 1% and calcium carbonate 0.2% was used. As theproduction medium, a medium comprising modified starch 6%, corn steepliquor 6% and potassium dihyorogenrphosphate 0.1% was used.

A 500-ml conical flask containing 100 ml of said preculture medium wassterilized by autoclaving at 120° C. for 20 minutes. After cooling toroom temperature, the flask was inoculated with 1˜2 loopfuls of an agarplate culture of Oidiodendron tenuissimum IFO 6798 and incubated at 25°C. for 4 days to prepare a seed culture. Then, a 500 ml conical flaskcontaining 100 ml of said production medium was sterilized byautoclaving at 120° C. for 20 minutes and cooled to room temperature,and FR901379 Substance was aseptically added at a final concentration of0.1%. The flask was then inoculated with 5 ml of said seed culture, andshake culture was carried out at 25° C. for 4 days to provide an enzymebroth.

EXAMPLE 1-6

Production of the acylases elaborated by subcultured strains belongingto the genus Oidiodendron

Using the following subcultured strains belonging to the genusOidiodendron as allotted from Institute for Fermentation, Osaka(2-17-85, Juso-Hommachi, Yodogawa-ku, Osaka), enzyme broths could beobtained according to a similar manner to that of Example 1-1 just as inthe case of Oidiodendron sp. No. 30084.

Oidiodendron echinulatum IFO 31963

Oidiodendron truncatum IFO 9951

Oidiodendron truncatum IFO 31812

EXAMPLE 2

Purification of the acylase elaborated by Oidiodendron tenuissium IFO6798

The enzyme fermentation broth obtained in Example 1-3 was adjusted to pH3 and centrifuged at low temperature. The resulting supernatant waspassed through an SP207 column. The effluent was filtered through a UFmembrane (Asahi Chemical Industry, AIP-1010) into 20 mM Tris-HCl buffer(pH 7). This solution was applied onto a DEAE-Toyopearl column (Tosoh,Cl⁻form), and elution was carried out with 20 mM citrate buffer pH5).After the active fraction was adjusted to pH 4, 0.6 M equivalent of(NH₄)₂SO₄ was added and dissolved, and the solution was further appliedonto a Phenyl-Topopearl column (Tosoh) eluting with 0.2 M(NH₄)₂SO₄-containing 20 mM citrate buffer (pH 4). The active fractionwas desalted and concentrated using a DF membrane (Asahi ChemicalIndustry, SIP-0013). The desalted concentrate was subjected to gelpermeation chromatography on a YMC-Diol column (YMC) (mobile phase: 0.1M NaCl-50 mM acetate buffer, pH 5). The purified acylase was subjectedto SDS-PAGE. As a result, the enzyme converged into a band correspondingto about 40 kD. The molecular weight of the acylase as determined by gelfiltration-HPLC with TSKgel G3000PWXL (Tosoh) was about 150 kD. Thoseresults suggested that the acylase is an enzyme protein of about 150 kDhaving identical or different subunits of about 40 kD.

The HPLC comprising a variable wavelength UV detector, a pump, and anintegrator was used. As the column, a TSK gel G3000 PWXL column (7.8 mmI.D.×30 cm) was used. Using a mobile phase consisting in 0.1 M phosphateere (pH 6)−0.3 M NaCl, the enzyme protein was eluted at a flow rate of0.5 mL/min. The molecular weight markers were chymotrypsinogen A (25kD), ovalbumin (43 kD), albumin (67 kD) and aldolase (158 kD). Theretention time under the above conditions was about 17.9 minutes and byreference to a calibration curve constructed with the markers, itsmolecular weight was estimated to be about 150 kD.

The process for deacylating the acyl side chain of the antifungal cycliclipopeptide compound (e.g. FR901379 Substance) which comprises the useof the acylase according to the invention is now described in detail.

This acyl side chain deacylation process was carried out by adding thefermentation broth obtained as above to the cyclic lipopeptide compound(e.g. FR901379 Substance) and incubating the mixture at a reactiontemperature of 20° C. to 50° C. and a pH level of about 2 to 6, anddetecting and separating the resulting cyclic peptide (e.g. FR179642Substance) by high performance liquid chromatography (HPLC).

The following examples are intended to specifically illustrate but by nomeans delimit the deacylation technology of this invention.

EXAMPLE 3-1

To 7 ml of the fermentation broth of Oidiodendron sp. No. 30084 obtainedin Example 1-1 was added 1 ml of an aqueous solution (20 mg/ml) ofFR901379 Substance (20 mg as FR901379 Substance; 16.7 μmol) as well as 2ml of a buffer (0.2 M sodium citrate buffer, pH 4.0), and the reactionwas carried out at 30° C. for 3 hours. The reaction was hen stopped byadding 0.4 M trichloroacetic acid and centrifuged at low speed to removeprecipitated high molecular weight protein and other impurities. TheFR179642 Substance produced was subjected to HPLC and monitored at 210nm to determine the acylase activity.

The HPLC comprised of a variable wavelength UV detector (HitachiL-4000), a pump (Hitachi L-6000) and an integrator (Hitachi D-2500) wasused. As the stationary phase, LiChrospher 100RP-18 (250 mm×4 mm i.d.,particle dia. 5 mm) was used. Using a mobile phase consisting in5-acetonitrile/0.5% ammonium dihydrogenphosphate, FR179642 Substance waseluted at a flow rate of 1 ml/min. The retention time of FR179642Substance was about 6.3 minutes. The yield of FR179642 Substance ascalculated from the data was 4.5 mg (4.8 μmol).

EXAMPLE 3-2

To 7 ml of the fermentation broth of Verticillium sp No. 30085 obtainedin Example 1-2 was added 1 ml of an aqueous solution (20 mg/ml) ofFR901379 Substance (20 mg as FR901379 Substance/ml; 16.7 μmol) as wellas 2 ml of a buffer (0.2 M sodium citrate buffer, pH 4.0), and thereaction was carried out at 30° C. for 1 hour. The reaction was thenstopped with 0.4 M trichloroacetic acid, and the mixture was centrifugedat low speed to remove high molecular weight protein and otherimpurities as a precipitate. The supernatant was subjected to HPLC andthe product FR179642 Substance being monitored at 210 nm to determinethe acylase activity.

The HPLC comprised of a variable wavelength UV detector (HitachiL-4000), a pump (Hitachi L-6000) and an integrator (Hitachi D-2500) wasused. As the stationary phase, LiChrospher 100RP-18 (250 mm×4 mm i.d.,particle dia. 5 mm) was used. Using a mobile phase consisting in 5%acetonitrile/0.5% ammonium dihydrogenphosphate, FR179642 Substance waseluted at a flow rate of 1 ml/min. The retention time of FR179642Substance was about 6.3 minutes. The yield of FR179642 Substance ascalculated from she data was 7 mg (7.5 μmol).

EXAMPLE 3-3

To 50 μl of the enzyme broth prepared by the procedure described inExample 2 was added 100 μl of an aqueous solution (100 mg/ml) ofFR901379 Substance (10 mg as FR901379 Substance/ml; 8.35 μmol) as wellas 100 μl of methanol, 100 μl of a buffer (0.5 M citrate buffer, pH 4)and 650 μl of water, and the reaction was carried out at 30° C. For 30minutes. The reaction was stopped by adding 1 ml of 4% acetic acid and 2ml of methanol, and the reaction mixture was subjected to HPLC. Theproduct FR179642 Substance was monitored at 215 nm, and the acylaseactivity was determined. The HPLC was comprised of a variable wavelengthUV detector (Shimadzu SPD-10A), a pump (Shimadzu LC-10AD) and anintegrator (Shimadzu C-R6A), and as the stationary phase, Kaseisorb LCPOSuper (200 mm×4.6 mm i.d., Tokyo Kasei) was used. Using 4% methanol/0.1%phosphoric acid at 40° C. as the mobile phase, FR179642 Substance waseluted at a flow rate of 1.2 ml/min. The retention time of FR179642Substance was about 6 minutes. The yield of FR179642 Substance ascalculated from the data was 400 μg (0.43 μmol).

EXAMPLE 3-4

To 50 μl of the enzyme solution as purified by the procedure describedin Example 2 was added 100 μl of a solution of Echinocandin B substance(in dimethyl sulfoxide, 100 mg/ml) (10 mg as Echinocandin Bsubstance/ml) as well as 100 μl of a buffer (0.5 M citrate buffer, pH 4)and 750 μl of water, and the reaction was carried out at 30° C. for 30minutes. The reaction was stopped by adding 1 ml of 4% acetic acid and 2ml of methanol, and the product Echinocandin B nuclear substance wasassayed by HPLC. The HPLC used was comprised of a variable wavelength UVdetector (Shimadzu SPD-10A), a pump (Shimadzu LC-10AD) and an integrator(Shimadzu C-R6A), and using LiChrosphr 100RP-18(e) (250 mm×4 mm i.d.,particle dia. 5 μm, E. Merck) as the stationary phase and 5%acetonitrile/0.5% ammonium phosphate at 40° C. as the mobile phase,Echinocandoin B nuclear substance was eluted at a flow rate of 10.0ml/min. The retention time of Echinocandin B nuclear substance was about6 minutes The yield of Echinocandin B nuclear substance as calculatedfrom the data was 3.1 μg (0.004 μmol).

EXAMPLE 3-5

To 50 μl of the enzyme solution as purified in Example 2 was added 100μl of a solution of Aculeacin A (in dimethyl sulfoxide, 100 mg/ml) (10mg as Aculeacin A substance/ml) as well as 100 μl of a buffer (0.5 Mcitrate buffer, pH 4) and 750 μl of water, and the reaction was carriedout at 30° C. for 30 minutes. The reaction was stopped by adding 1 ml of4% acetic acid and 2 ml of methanol, and the product Aculeacin A nuclearsubstance (=Echinocandin B nuclear substance) was assayed by HPLC. TheHPLC was comprised of a variable wavelength UV detector (ShimadzuSPD-10A), a pump (Shimadzu LC-10AD) and an integrator (Shimadzu C-R6A)and using LiChrospher 100RP-18(e) (250 mm×4 mm i.d., particle dia. 5 μm,E.Merck) as the stationary phase and 5% acetonitrile/0.5% ammoniumphosphate at 40° C. as the mobile phase, Aculeacin A nuclear substancewas eluted at a flow rate of 1.0 ml/min. The retention time of AculeacinA nuclear substance was about 6 minutes. The yield of Aculeacin Anuclear substance as calculated from the data was 17.7 μg (0.022 μmol).

EXAMPLE 3-6

To 700 μl of the fermentation broth obtained by using Oidiodendrontruncatum IFO 9951 in Example 1-4 was added 100 μl of an aqueoussolution (100 mg/ml) of FR901379 Substance (10 mg as FR901379Substance/ml; 8.35 μmol) as well as 200 μl of a buffer (0.2 M citratebuffer, pH 4), and the reaction was carried out at 30° C. for 60minutes. The reaction was stopped by adding 1 ml of 4% acetic acid and 2ml of methanol, and the mixture was filtered through a membrane filter(0.45 μm) to remove high molecular weight protein and other impurities.The filtrate was subjected to HPLC and the product FR179642 Substancewas monitored at 215 nm to determine the acylase activity.

The HPLC was comprised of a variable wavelength UV detector (ShimadzuSPD-10A), a pump (Shimadzu LC-10AD) and an integrator (Shimadzu C-R6A),and using Kaseisorb LC PO Super (200 mm×4.6 mm i.d., Tokyo Kasei) as thestationary phase and 4% methanol/0.1% phosphoric acid at 40° C. as themobile phase, the product FR179642 Substance was eluted at a flow rateof 1.2 ml/min. The retention time of FR179642 Substance was about 6minutes. The yield of FR179642 Substance as calculated from the data was232 μg/ml (0.25 μmol/ml).

EXAMPLE 3-7

Using he procedure described in Example 3-6, FR179642 Substance could beobtained from the culture of Oidiodendron truncatum IFO 31812 asobtained in Example 1-4 as well. The calculated yield of FR179642Substance was 266 μg (0.28 μmol).

EXAMPLE 3-8

Using the procedure described in Example 3-6, FR179642 Substance couldbe obtained from the culture of Oidiodendron echinulatum IFO 31963 asobtained in Example 1-4 as well. The calculated yield of FR179642Substance was 136 μg (0.15 μmol).

The characteristics of the process of deacylation of the acyl side chainof an antifungal cyclic lipopeptide compound (e.g. FR901379 Substance)by the fungal acylase are now described.

The data presented were generated by the experimental proceduresdescribed in Example 3-1 through Example 3-5 with modification ofconditions such as the buffer (0.2 M˜0.5 M sodium citrate buffer,potassium phosphate buffer, and Tris-HCl buffer in suitablecombinations), the reaction temperature, and the concentration ofpotassium chloride added. The acylase activity was expressed in theconcentration (determined by HPLC) of FR179642 Substance or EchinocandinB nuclear substance at completion of the reaction.

Optimum Reaction pH

Test Example 1-1

The optimum pH for the acylase elaborated by Oidiodendron sp. No. 30084

The influence of reaction pH on the concentration of FR179642 Substanceat completion of the reaction was studied using the same procedure asExample 3-1. The results are shown in Table 3.

TABLE 3 Concentration of FR179642 Substance at pH completion of reaction(μg/ml) 3 590 4 450 5 210 6  70 7  −5* 8  −2* 9  0 *caused bymeasurement error

EXAMPLE 1-2

The optimum pH for the acylase elaborated by Verticillium sp. No. 30085

The influence of reaction pH on the concentration of FR179642 Substanceat completion of the reaction was studied using the same procedure asExample 3-2. The results are shown in Table 4.

TABLE 4 Concentration of FR179642 Substance at pH completion of reaction(μg/ml) 3 480 4 520 5 410 6 100 7  10 8   −10* 9   −20* *caused bymeasurement error

The above results indicate that, in the working of the invention, theoptimum reaction pH is 2 to 6, preferably 3 to 5, for both acylases.

Test Example 1-3

The optimum pH for the acylase elaborated by Oidiodendron tenuissimumIFO 6798

The influence of reaction pH on the concentration of FR179642 Substanceat completion of the reaction was studied using the same procedure asExample 3-3. The results are shown In Table 5.

TABLE 5 Concentration of FR179642 Substance at pH completion of reaction(μg/ml) 2 434 3 422 4 366 5 312 6 65 7 0 8 0

Test Example 1-4

The optimum pH for the acylase elaborated by Oidiodendron tenuissimumIFO 6798

The influence of reaction pH on the concentration of Echinocandin Bnuclear substance at completion of the reaction was studied using thesame procedure as Example 3-4. The results are shown in Table 6.

TABLE 6 Concentration of Echinocandin B nuclear pH substance atcompletion of reaction (μg/ml) 2 2.5 3 2.8 4 2.6 5 1.4 6 0.16 7 0.17 80.14

Regardless or substrates, the reaction was considerably retarded in theneutral and higher pH range. When FR901379 was used as the substrate,the reaction rate increased with declining pH. When Echinocandin B wasused as the substrate, high reaction rates were obtained within the pHrange of 2˜4.

The above results (Test Examples 1-3 and 1-4) indicate that withwhichever of the substrates, the optimum reaction pH is 2˜6, mostpreferably 2˜4. It is also clear that the reaction does notsubstantially proceed in the neutral and higher pH region.

Optimum Reaction Temperature

Test Example 2-1

The optimum temperature for the acylase elaborated by Oidiodendron sp.No. 30084

The influence of reaction temperature on the concentration of FR179642Substance at completion of the reaction was studied using the procedureof Example 3-1. The results are shown in Table 7.

TABLE 7 Concentration of FR179642 Substance at Temperature completion ofreaction (μg/ml) 20 190 25 280 30 460 35 550 40 600 45 — 50 280

Test Example 2-2

The optimum temperature for the acylase elaborated by Verticillium sp.No. 30085

The influence of reaction temperature on the concentration of FR179642Substance at completion of the reaction was studied using the procedureof Example 3-2. The results are shown in Table 8.

TABLE 8 Concentration of FR179642 Substance at Temperature completion ofreaction (μg/ml) 20 250 25 470 30 700 35 — 40 780 45 — 50 440

The above results indicate that for both acylases the optimum reactiontemperature is 20≠50° C., preferably 30˜40° C.

Test Example 2-3

The optimum temperature for the acylase elaborated by Oidiodendrontenuissimum IFO 6798

The influence of reaction temperature on the concentration of FR179642Substance at completion of the reaction was studied using the procedureof Example 3-3. The results are shown in Table 9.

TABLE 9 Concentration of FR179642 Substance at Temperature completion ofreaction (μg/ml) 25 243 30 383 35 606 40 828 45 379 50 80 55 30 60 22

Test Example 2-4

The optimum temperature for the acylase elaborated by Oidiodendrontenuissimum IFO-6798

The influence of reaction temperature on the concentration ofEchinocandin B nuclear substance at completion of the reaction wasstudied using the same procedure as Example 3-4. The results are shownin Table 10.

TABLE 10 Concentration of Echinocandin B nuclear Temperature substanceat completion of reaction (μg/ml) 25 1.8 30 2.7 35 4.2 40 4.8 45 3.2 500.5 55 0.3 60 0.2

Regardless of substrates, the reaction proceeded satisfactorily at25˜45° C. and the highest reaction rate was obtained at 40° C.

Results of Addition of a Solvent to the Reaction System

Test Example 3-1

The effect of addition of methanol to the reaction system involving theacylase elaborated by Oidiodendron tenuissimum IFO 6798

The effect of addition of methanol to the reaction system on theconcentration of FR179642 Substance at completion of the reaction wasstudied using the procedure of Example 3-3. The results are shown inTable 11.

TABLE 11 Concentration of Concentration of FR179642 Substance methanol(%) at completion of reaction (μg/ml) 0 273 5 360 10 400 20 407 30 33240 69 50 0

Test Example 3-2

The effect of addition of dimethyl sulfoxide to the reaction system onthe concentration of Oidiodendron tenuissimum IFO 6798

The effect of addition of dimethyl sulfoxide to the reaction system onthe concentration of Echinocandin B nuclear substance at completion ofthe reaction was studied using the procedure of Example 3-4. The resultsare shown in Table 12.

TABLE 12 Concentration Concentration of Echinocandin B of dimethylnuclear substance at completion sulfoxide (%) of reaction (μg/ml) 0n.t.* 5 2.8 10 3.1 20 3.8 30 3.5 40 1.0 50 0.1 *n.t. = not tested

When FR901379 was used as the substrate, the reaction rate was increasedin the presence of 10-20% of methanol. When Echinocandin B was used asthe substrate, the reaction rate was increased on addition of 20˜30%, ofdimethyl sulfoxide.

Influence of Salt Concentration

Test Example 4-1

The influence of salt (KCl) concentration on the reaction involving theacylase elaborated by Oidiodendron tenuissimum IFO 6798

The influence of salt (KCl) concentration in the reaction system on theconcentration of FR179642 substance at completion of the reaction wasinvestigated using the procedure of Example 3-3. The results are shownin Table 13.

TABLE 13 Concentration Concentration of FR179642 Substance of KCl (M) atcompletion of reaction (μg/ml) 0 369 0.3 352 0.6 336 0.9 343 1.2 317 1.5326 1.8 315

Test Example 4-2

The influence of salt (KCl) concentration on the reaction involving theacylase elaborated by Oidiodendron tenuissimum IFO 6798

The influence of salt (KCl) concentration in the reaction system on theconcentration of Echinocandin B nuclear substance at completion of thereaction was investigated using the procedure of Example 3-4. Theresults are shown in Table 14.

TABLE 14 Concentration of Echinocandin B Concentration nuclear substanceat completion of KCl (M) of reaction (μg/ml) 0 2.7 0.3 2.2 0.6 2.1 0.92.1 1.2 2.0 1.5 1.7 1.8 1.7

The as or of KCl had no effect.

It can be estimated from the above data that Km is 1590 μM and Vmax 4.2U/mg-protein when the reaction is carried out using FR901379 Substanceas the substrate under the conditions of reaction temperature=40° C.,reaction pH=3 and reaction time=15 minutes. The amount of the enzymeyielding 1 μmol of FR179642 Substance per minute was taken as 1 U.

The cyclic lipopeptide acylase obtainable by growing anacylase-producing strain belonging to the genus Oidiodendron isspecifically described below. Characteristics of the acylase derivedfrom Oidiodendron tenuissimum IFO 6798

1) Activity:

The enzyme catalizes deacylation of the fatty acyl moiety of a cycliclipopeptide compound represented by FR901379 Substance and FR901379analogs such as Echinocandin B, Aculeacin A, etc.

2) Optimum pH: pH 2≠4

3) Optimum range of temperature for action: 25≠45° C.

4) Inhibition, activity and stabilization:

Methanol: concentration-dependent activity up to 20% in the reactionmixture and inhibition at and over 40%.

5) molecular mass:

It is considered to be an enzyme protein of about 150 kD which hasidentical or different subunits of about 40 kD.

6) Vmax and Km values

Km is 1590 μM and Vmax is 4.2 U/mg-protein when determined usingFR901379 Substance as the substrate under the conditions of reactiontemperature=40° C., reaction pH=3 and reaction time=15 minutes,

7) Substrate specificity

The deacylating activities for Echinocandin B and Aculeacin assubstances are less potent than the activity for FR901379.

Coleophoma sp. F-11899 which elaborates FR901379 Substance and thefungal strain Oidiodendron sp. No. 30084 and fungal strain Verticilliumsp. No. 30085, both of which are producers of the acylase of theinvention, have been deposited with National Institute of Bioscience andHuman Technology (NIBH, Higashi 1-1-3, Tsukuba-shi, Ibaraki, Japan).

Microorganism Accession No. Coleophoma sp. F-11899 FERM BP-2635Oidiodendron sp. No. 30084 FERM BP-5943 Verticillium sp. No. 0085 FERMBP-5944

What is claimed is:
 1. A process for producing a cyclic peptide compoundof the following formula (II):

or a salt thereof, which comprises contacting a cyclic lipopeptidecompound of the following formula (I):

or a salt thereof in an aqueous solvent with a crude or purified enzymesolution, which is prepared by culturing Oidiodendron echinulatum IFO31963, Oidiodendron tenuissimum IFO 6798, Oidiodendron truncatum IFO9951, or Oidiodendron truncatum IFO 31812 in the presence of a cycliclipopeptide compound; wherein R¹ is acyl; R² is hydroxyl or acyloxy; R³is hydrogen or hydroxyl; R⁴ is hydrogen or hydroxyl; R⁵ is hydrogen orhydroxysulfonyloxy; and R⁶ is hydrogen or carbamoyl.
 2. The process ofclaim 1, wherein R⁵ is hydroxysulfonyloxy, and R⁶ is carbamoyl.